- Email: [email protected]
Complete synthesis and transcription in vitro of a gene coding for human ribosomal 5S RNA
Gene. 64 (1988) 77-85
77
Elsevier GEN 02332
Complete synthesis and transcription (Ribosomal
5s RNA;
III-transcription
in vitro of a gene coding for human rihosomal 5s RNA
gene expression;
in vitro transcription;
HeLa cell extract;
RNA polymerase
III;
Pol
factors)
Edgar Wingender”, Ronald Franka, Helmut Bliicker”, Lingru Wang b, Dieter Jahnb and Klaus H. Seifart’ ‘I Gesellschaft ftir Biotechnologische Forschung, D-3300 Braunschweig (F. R. G.) Tel. 0531/6181206. biologic und Tumorforschung, Philipps-Universitiit, D-3550 Mmburg (F.R. G.) Received
17 November
Accepted
4 December
1987
Received
by publisher
12 January
and Institut ftir Molekular-
1987 1988
SUMMARY
The gene coding for the major human ribosomal 5s RNA was chemically synthesized and cloned into a pUC13 vector. This approach was taken, because attempts to isolate the human 5S gene have thus far yielded either pseudogenes or variant 5s genes of unknown function. The synthetic human gene was transcribed by RNA polymerase III either in a crude HeLa cell extract or in a system reconstituted from partially purified transcription factors. Comparative studies with the Xenopus luevis somatic 5s gene show that the human gene is transcribed with similar fidelity and an efficiency of about 80% under optimal conditions. The time-course of transcription and optimal concentrations of template and transcription factors were found to be similar for both genes studied. The synthetic gene described may prove useful to study its interaction with human transcription
factors
in a homologous
system.
INTRODUCTION
Transcription of the gene for 5s rRNA by RNA polymerase III has proven to be an extremely useful
Correspondence to: Dr. K.H.
Seifart,
biologie und Tumorforschung,
Karl-von-Frisch-Strasse,
Marburg
(F.R.G.)
Abbreviations:
bp, base pair(s); liquid
deoxynucleotide; PMSF,
D-3550
DNA coding
h, human;
polyacrylamide fluoride;
for 5S RNA;
RNA.
I’)88 El.xGx
HEPES.
sulfonic acid; HPLC,
chromatography;
PAGE,
037X-l 119!88~$03.50 0
DTT, dithiothreitol;
N’-2-ethane
phenylmethylsulfonyl
5S DNA,
Rir Molekular-
Tel. 06421-285013.
hydroxyethylpiperazine performance
Institut
oligo,
higholigo-
gel electrophoresis;
TF, transcription 5S rRNA,
factor;
ribosomal
5S
model for the characterisation of the transcription factors involved and for the development of concepts regarding the mechanism of gene regulation in eukaryotic cells. Simultaneously it has become increasingly apparent that the development of homologous systems may be essential for the appropriate characterisation of promoter sequences and factors interacting with them. While TF IIIA, IIIB and IIIC have been isolated and partially purified from human cells (Segall et al., 1980; Wingender et al., 1986; Boulanger et al., 1987) the homologous gene for 5s rRNA has hitherto not been isolated in a transcriptionally active form from genomic DNA. A DNA sequence from a human library, which hybridized to 5s RNA and bound to
Science Publlshcrs B.V. (Bmmcdical Dwision)
78
TF IIIA was not transcribed change in the internal Roeder,
in vitro, due to a base
control
region (Emerson
1984) and it possibly
represents
of a large family of pseudogenes, of unknown
function
(Doran
and
a member
or variant
5S genes
et al., 1987).
In view ofthe outlined necessity to obtain a human 5s rRNA
gene of correct
ficulties associated
library, we synthesized for
the
major
Weissman, homologous
sequence
with its isolation a nucleotide
human
5s
1967) to investigate
and
factors
denaturing
temperatures
conditions
and ligated at
with T4 DNA ligase.
Finally the reaction
products
were checked
by PAGE
(see Fig. 2); all this according
procedures
detailed
elsewhere
(Frank
again to the
et al., 1983;
1987). (b) Cloning and sequencing
sequence coding
rRNA
(Forget
and
its transcription
by a
involved.
Expression of chemically synthesized eukaryotic genes in eukaryotic cells or cell extracts has been hitherto restricted to a few examples of synthetic structural genes due to the complicated and often unknown structure of their promoters. To express a synthetic human interferon-a, gene in murine cells, e.g., these problems were partially circumvented by using a heterologous viral promoter (Coulombe and Skup, 1986). Genes transcribed by RNA polymerase III, however, harbour their own promoters inside the transcribed region. Here we present results showing that a synthetic human 5S rRNA gene is correctly and productively transcribed in an in vitro system reconstituted from a HeLa cellular extract. This proves that for the expression of the human 5S RNA gene, 5’-flanking sequences are not essential, although they might exert additional regulating influences.
MATERIALS
under
the dif-
from a human
cell extract, and to study its interaction
with the transcription
PAGE elevated
AND METHODS
Using
the single-stranded
double
strand
BumHI
protruding
that
were
ends of the synthetic designed
as Sal1
ends, respectively,
gene was cloned into a pUCl3
and
the synthetic
vector. After ligation,
the plasmid was transfo~ed into ~,~~~e~ic~ja coli strain BMH 7 I-18, white clones were selected and checked by restriction analysis. Inserts from the plasmid DNA of positive clones were excised with Hind111 + EcoRI, recloned into phage M13mp18 and sequenced according to Sanger et al. (1977). (c) Preparation of DNA and cellular extracts Biochemicals were reagent grade from Boehringer Mannheim. The plasmids used in this study were isolated in their superhelical form as described (Currier and Nester, 1976) and purified by sucrose density gradient centrifugation. Plasmids pH5S and pX ls5S contained single copies of the synthetic human 5S gene and the X. laevis somatic 5S gene in pUC13 (2797 bp) and pUC I9 (2884 bp), respectively. The cytoplasmic HeLa cell extract (SIOO) was prepared from 20 liter suspension cultures with the titer of 4-5 x lo5 cells/ml, as described previously (Gruissem et al., 1981), and contained approx. 15 mg proteiniml.
(a) Gene design and synthesis Oligodeoxynucleotides comprising basically the coding sequence of the human 5S rRNA, its complementary strand, and ‘sticky ends’ for the restriction enzymes Sal I and BamHI were designed with the SYNGEN option of the GENMON computer programme package (see Fig. 1). synthesised with cellulose disks as segmental supports, purified after deprotection over reversed-phase (disposable cartridges) and ion-exchange (HPLC) materials, labelled at their 5 ’ -termini with [ y-‘*PI ATP and T4 polynucleotide kinase, analysed by sizing on a 20”,
(d) In vitro synthesis and electrophoretic RNA
analyses of
The in vitro transcription reaction mixtures were incubated at 30°C for 1 h unless stated otherwise and contained in a total volume of 50 11 0.025 mM and 10 /iCi [ z-~‘P] GTP (440 Ci/mmol, Amersham), 0.5 mM each of ATP, UTP and CTP 20 mM Tris ’ HCI, pH 7.9, 60 mM KCl, 5 mM MgClz, 3 mM DTT, IO?,; (v/v) glycerol, variable amounts of plasmid DNA and 15 ~1 SlOO. The in vitro transcription products were purified
19
and analyzed acrylamide
by PAGE, gels, and
using 7 M urea-lo”/:, subsequent
poly-
135 or 150 mM
autoradiography
through
overnight as described (Gruissem and Seifart, 1982). The region of the gel containing the RNA was excised
tions fractions
and quantitated
through,
by Cerenkov
radiation.
of transcription
All operations stated
were performed
otherwise.
transcription of HeLa
For
unless
of individual
trated by ammonium
culture
against
(about
B and
stored
at
in preparation).
two consecutive steps of buffer I containing 0.35 M KC1 (fraction B; approx. 1.3 mg protein~ml) and 0.6 M KC1 (fraction C; approx. 0.5 mg protein/ml). Fractions B and C contain TFIIIB and TFIIIC, respectively, and both fractions contain RNA polymerase III. The enzyme was removed from these fractions by dialysing against buffer II (20 mM Tris +HCI, pH 7.9,5 mM MgCl,, 3.0 mM DTT and 0.2 mM PMSF) containing 20% glycerol and either
RESULTS
AND DISCUSSION
(a) Gene synthesis The
chemical
and cloning synthesis
of oligos
as building
blocks for a relatively long DNA duplex comprising a complete gene is most efficiently carried out by simultaneous synthesis of adjacent fragments of
30 I
40 I
3
1
and
dialysed
60 mM KC1 and IO?/;, - 80°C. Human TFIIIA
(hTFIIIA), contained in fraction A (see above) was purified by additional chromatographic steps involving rechromato~aphy on phosphocellulose as will appropriately be published elsewhere (L. W., R. Waldschmidt, D. J., E. W. and K.H. S., manuscript
washed with the same buffer and the flow-through was collected (fraction A; approx. 3.0 mg protein/ml). The column was subsequently eluted with
20 I
sulfate precipitation,
buffer II containing
glycerol
pH 7.9, 3.0 mM DTT, 0.2 mM PMSF, 20% glycerol) containing 0.1 M KCl. The column was
I
III is retained
(Segall et al., 1980). Fractions
at 0-4°C
in suspension
10
RNA-polymerase
in the flow-
nation and from RNA polymerase III, but contained several other proteins. These fractions were concen-
15 mg protein/ml) was applied to a 30 ml; 2.6 x 10 cm phosphocellulose column (Whatman Pl I in its sodium form) in buffer I(20 mM HEPES,
I
bed
Under these condi-
B and C are contained
whereas
passage
C were assayed to be free of mutual cross contami-
the isolation
1
and
protein/ml
factors
factors the SIOO extract from 25 liters
cells grown
sulfate, (1 mg
volume) at these ionic strengths.
on the column (e) Fractionation
~monium
DEAE-Sephadex
50 I
60 I
5
7
TCGACGTCTACGGCCATACCACCCTGAACGCGCCCGATCTCGTCTGATCTC(S’WXT~T~ -TGCCGGTATGGTGGGACTTGCGCGGGCTAGAGCAGACTAGAGCCTTCGAl-KGT2
4
70
80
I
I
90
1
100
110
I
I
11
9 GCCTGGTTAGTACTTWTGGGAGA
..
6
120
I 15
13
CCGCCTGGGMTACCGGGTGCTGTAGGCTTTTAGACTlTTG
CGGACCAATCATGAACCTACCCTCTGGCGGACCCTTATGGCCCACGACATCCGAAAATCTGAAAACCTAG 0
10
Fig. I. Synthesis S. horedis position Sequence
of the human
termination
sequence
5S rRNA gene. Both strands and a BantHI
in the DNA duplex). The overlappings numbering
refers to the transcription
14
12 of the gene for human
site complement
were synthesised
of complementary start point
( = 1).
segments
5S rRNA
as adjacent
were optimised
flanked fragments
by a Sal1 site complement, (numbered
using a computer
according
programme
an
to their
(SYNGEN).
each strand which cover the complete sequence. For optimal hybridisation of complementary fragments
play only a single deviation
prior to their ligation, they have to be properly defined to achieve most stable and unique overlaps.
center
This was achieved the
computer
using an option
programme
package
which runs on VAX computers the operating (Frank For
(SYNGEN)
here, the nontranscribed
structed
of seven,
the transcribed
oligos (Fig. 1). These
fragments
53 which is located
and has recently
been shown
in the
(Pieler et al., 1987) to be important
for
GENMON
and IBM-PC
human
reported
in position
of the boxA homologue
con-
of
SS rRNA strand strand
/
under
systems VMS and DOS, respectively
et al., 1987). synthesis of the
trol region
within the internal
A
I
8
gene
was conof eight
were synthesized
using the filter method, purified and processed as described (Frank et al., 1983; 1987). Analysis of the individual oligos by gel electrophoresis revealed some minor contaminations in an overexposed autoradiograph (Fig. 2A). Nevertheless, they can be efficiently ligated to the correct product in a single reaction step (Fig. 2B) due to their proper design allowing ligation at elevated temperature and, thereby, suppressing any side-reactions. Referring to the nontranscribed strand, the 5’ terminus of the gene was designed to be compatible to a SulI restriction site. The subsequent region coding for the human 5s RNA was taken from the known RNA sequence (Forget and Weissman, 1967; Erdmann and Wolters, 1986). At the 3’ end of this region, the transcription termination sequence of a Xenopus borealis 5s rRNA gene (oocyte-type gene 1; Korn and Brown, 1981) was added which comprises two clusters of four thymidine residues each. These short T-stretches have been shown to represent efficient termination signals for RNA polymerase III transcription (Bogenhagen and Brown, 1981). The 3’ terminus consists of a sequence compatible to a BarnHI restriction site. Thus, the 5s rRNA gene complemented by a termination sequence was suitable to be cloned between the ScllI and the BumHI sites of the vector pUC13 (Messing, 1983). Subsequently, the synthetic gene sequence was verified using the sequencing method of Sanger et al. (1977). This sequence was compared to other 5s RNA genes previously employed for in vitro transcription studies, i.e., the oocyte-type 5s RNA gene from X. borealis (Korn and Brown, 1981) and theX. luevis somatic 5s gene (Brownlee et al., 1972; Fig. 3). The X. Iuevis somatic and the synthetic human gene dis-
m 234m 194mD
'
118c,
721)
1 Fig. 2. (A) Sizing of the synthetic
oligos (in the order
from left to right) on a 20”, polyacrylamide urea; lanes: A, the A ladder
starting
starting
of the one-step
with T,. (B) Analysis
to I5 on a IO”,, non-denaturing sample
of the crude ligation
4O”C, I h at 37”C, markers,
7M
with A,: T, the T ladder ligation of oligos I
polyacrylamide
mixture
I to 15
gel containing
gel; laws:
after incubation
1h at 3O’C, and overnight
(5’-“P-labelled
2
HueHI-fragments
for
I,
I h at
at 15’C; 2, M,
of 4x174).
81
1
20
10
hwn 5s RNA
GTCTACGGCCATACCACCCTGAACGCGCCCGATCTCGTCT l l ******** *********** l l *************
Xls
GCCTACGGCCACACCACCCTGAAAGTGCCCGATCTCGTCT
5s RNA
60
70
80
Xbo 5s RNA
GATCTCGGAAGCGATGCAGGGCCGGGCCTGGTI-AGTACCT l *********** * l ***** ********a****** l
hum 5s RNA
GATCTCGGAAGCTAAGCAGGGTCGGGCCTGGlTAGTACTT l *********** ***************************
Xls
GATCTCGGMGCCAAGCAGGGTCGGGCCTGGlTAGTAClT
5s RNA
90
110
100
120
Xbo 5s RNA
GGATGGGAGACCGCCTGGGAATACCAGGTGTCGTAGGCl-T l ************************ **** ********
hum 5s RNA
GGATGGGAGACCGCCTGGGAATACCGGGTGCTGTAGGClT ******** ********a**************** ****
Xls
GGATGGGAGACCGCCTGGGAATACC
5s RNA
comparison Sequences
AGGTGTCGTAGGCTT
of the gene for human 5s RNA (hum 5s RNA) with the genes for X. borealis oocyte-specific 1981) and for X. laevis somatic
5s RNA; Korn and Brown, by an asterisk.
4.0
GCCTACGGCCACACCCCCCTGAAAGTGCCCGATCTCGTCT l l ******** *** l ****** * **************
50
Fig. 3. Sequence
30
Xbo 5s RNA
of the non-coding
strands
5s RNA (Xls 5s RNA; Brownlee
are given; numbering
et al., 1972). Identical
refers to the transcription
5s RNA (Xbo
residues
are marked
start point ( = 1).
transcription efficiency (McConkey and Bogenhagen, 1987). The oocyte gene promoter differs in this and two additional positions from both these somatic genes.
5s-
(b) Time course of the in vitro transcription of the Xenopus Zuevis somatic and synthetic human SS-genes by a HeLa cell extract A human genomic clone, containing the 5s RNA sequence with one base change in the internal control region was not transcribed in vitro (Emerson
0
J
1
8 2
3
10
5
6
template. times
represent
products
after 5, 10,20,30,45
20
30 Time
45 1min. 1
60
containing counting.
reactions
were stopped
were separated
gels and visualised 5s RNA
insert, part A) or human
*
of the X. /aeviy somatic 5s RNA gene (o--(>). with nucle-
labelled GTP and 20 pg/ml of the indicated
The transcription
and RNA
polyacrylamide l-6
human
HeLa cell extract (SlOO) was incubated
oside triphosphates, 4
for transcription
or the synthetic
Cytoplasmic
-Y
1:
5
Fig. 4. Time course (M)
by autoradiography.
synthesised synthetic
Lanes
from the X. luevis (upper
5s gene (lower insert, part B)
and 60 min, respectively.
5s RNA were excised
at different
on 7 M urea-lo”,
Radioactive
and quantified
bands
by Cerenkov
82
and Roeder, analyse human the
1984). It was therefore
the transcription gene described
established
capacity
of transcription
5s gene. As was previously
(Pelham
and Brown,
scription
of the latter gene displays
to
gene is transcribed product
of the synthetic
here and to compare
kinetics
X. laevis somatic
of interest
it with
Xenopus somatic
of the
thesis
shown
total synthesis
1980; Jahn et al., 1987) trana clear time-lag,
with similar fidelity, yielding
identical
in size to that synthesised
5s gene. The rates of RNA
from both
somewhat
genes
are comparable,
has repeatedly
lower
(about
Figs.
syn-
although
been observed
20%,
a
on the
to be
4 and
5) in
to the Xenopus gene. The reason for this
comparison
presumably due to the delayed incorporation of TFIIIB into the transcription complex (Bieker et al.,
is not clear, but could be attributed to the lack of flanking sequences, possibly modulating the tran-
1985). As shown in Fig. 4, the synthetic
scription
gene
is productively
transcribed
human
in a HeLa
5s cell
extract and the formation of 5s RNA displays a very similar time course, including the time-lag mentioned above. (c) Influence of template concentration To investigate whether the human 5s gene is accepted by transcription factors in the HeLa cell extract with comparable affinity, a DNA titration was conducted in comparison to theX. laevis somatic 5s gene. As is demonstrated
in Fig. 5 the human
ever,
efficiency
that
observed
the
of this gene. It is evident,
DNA-optimum
for transcription
how-
characteristically
of the
5s
gene
and
attributed to the individual dispersion of TFIIIA and TFIIIC to separate genes at high DNA concentration without formation of productive preinitiation complexes (Wingender et al., 1984), is similar for both genes investigated. The absolute position of this optimum is different from that observed for the oocyte-type 5s gene from X. borealis (Gruissem et al., 1981; Jahn et al., 1987). This might be due to several additional base exchanges in the promoter region (50-90) of the latter gene when compared to
l
\ \ 0
\ \ \ \
1
\ \
\ \
\ \
\ \
\ \
\
’\
‘1
‘. \ \\ \
’\
-
a.,
.”
d”
DNA Fig. 5. Transcription GTP and increasing and quantitation
dependency amounts
on template
ofX. luevis (M
were as described
concentration.
&-hnll
HeLa S 100 was incubated
and insert A) or synthetic
in the legend to Fig. 2.
-
for 1 h with nucleotide
human 5s DNA (o-_O
triphosphates,
and insert B). Product
labclled analysis
83
either the X. laevis somatic
or the synthetic
human
gene (Fig. 3) causing less stable protein-DNA
inter-
actions
(Wormington
et al., 198 1).
(d) Influence of TFIIIA Binding of TFIIIA
and TFIIIC
from HeLa cells
to the internal
control region of
the 5s gene is the primary event for the formation transcription
complexes
on this gene. Although
of the
exact function of TFIIIC in this context is still not fully understood, recent investigations by Pieler et al. (1987) have demonstrated
interactions
of this factor
with boxA and probably also with boxC of the internal control region. It was therefore important to analyse the effect ofthese factors on the transcription
Fig. 6. Titration stituted
of the synthetic human 55 gene. It was found (Fig. 6) that 5S RNA synthesis from both genes increases with rising concentrations ofhTFIIIA up to a certain point and then decreases with very high concen-
genes in question. A comparable optimum is not observed for the titration of hTFIIIC (Fig. 7). It was observed that rising hTFIIIC concentrations increased 5s RNA formation without a subsequent decline. As is shown in Fig. 7, maximal rates of 5S RNA synthesis are
Fig. 7. Titration
of increasing
amounts
RNA gene (part B). Transcription ofTFIll.A,
10.0 ,ul ofTFIIIB,
The amounts
of hTFIIIf
of hTFIItC
factors
in a reconstituted
were
purilied
AND
METHODS,
TFIIIC,
varying amounts
template
were incubated
hTFIIIA
employed
ofTFIIIC
amounts
of hTFIIIA
respectively.
from
HeLa
in a recon-
(part A) OF synthetic ceils
factors as
IIIA, IIIB
described
section e. Ten yl ofTFIIIB, ofTFIIIA for
in
IO ~1 of
and 10 p’g DNA/ml
of either
1h in all assays. The amounts
of
were: in part A (lanes 1-5) O.OS,O.I, 0.5. 1.0,
5.0 ~1, respectively,
and in part B (lanes l-4) 0.05,0.5,
Quantitation
I .O. 5.0 ~1,
of 5s RNA was as in Fig. 2.
possibly reached at lower concentrations of/zTFIIIC in the case of the Xenopus gene. Footprint analyses (not shown; manuscript in prep~ation) proved, however, that hTFIIIC has little or no effect on the affinity of hTFIIIA binding to the human gene.
system with the X. iuevis somatic
were purified from HeLa celis as described
varying concentrations employed
IIIC
MATERIALS
trations of hTFIIIA. The basic phenomenon is similar for both genes, although the exact position of the optimum is slightly different, which could indicate an altered interaction of this factor with the two
of increasing
with the X. lnevis somatic
5s RNA gene (part B). Transcription
human and
system
and 5 ,ugjml ofeither
in
MATERIALS
DNA template
were 0.1, 0.5, 1, 2.5, 5, 7.5. 10, 20 and 50~1 in lanes
l-9,
(part A) or synthetic AND
METHODS,
were incubated
respectively.
human
5s
section e. One iti for 1 h in all assays.
84
(e) Conclusions
ACKNOWLEDGEMENTS
A gene coding for the major human chemically
synthesized.
5S rRNA was
This gene deviates
X. luevis somatic 5s gene, frequently studies, in eight positions.
from the
used for in vitro
One of them (at position
53) is located within the A box of the internal
control
region (Pieler et al., 1987). Although in a degenerate position of the BoxA consensus sequence, derived from either the tRNA genes (Ciliberto eukaryotic
5s RNA sequences
is apparently
important
We
acknowledge
Deutsche
financial
support
Forschungsgemeinschaft
conducted
at the University
of
the
to the research
of Marburg
and the
expert technical assistance of Frauke Seifart, Ursula Kopiniak and Verena Buckow (Marburg) as well as Helga Krause,
Christiane
Giesa,
Wiebke
Heikens
and Heiko Mielke (Braunschweig).
et al., 1983) or
(Pieler et al., 1987), it
for transcription
efficiency
(McConkey and Bogenhagen, 1987). However, we did not observe enhanced transcription as reported by these authors for a CG-TA transition in that position of the X. borealis somatic 5s gene. Our results clearly show that the synthetic human 5S rRNA gene is correctly and efficiently transcribed by RNA polymerase III either in a crude HeLa cell extract or in a reconstituted system of partially purified transcription factors. This proves that flanking regions are not required for transcription of the human 5S gene as was previously shown for the X. borealis somatic gene (Bogenhagen et al., 1980; Sakonju et al., 1980). Nevertheless, these flanking sequences may exert either positively or negatively modulating influences, as has recently been shown for some point mutations in the upstream region of that gene by McConkey and Bogenhagen (1987). Differences in the flanking sequences between the genes compared in this study may account for the slightly lower transcription efficiency of the synthetic human gene (approx. 80% under optimal conditions) and may possibly overcome the otherwise positive C + T transition at position 53. The synthetic gene described may prove useful to study its interaction with human transcription factors in a homologous system. We are presently analysing whether the small differences observed in the factor concentrations required for optimal transcription of the two genes could reflect altered protein-DNA interactions. Preliminary results from comparative footprint experiments show an altered interaction of human TFIIIA with the human and X. laevis somatic 5S genes, respectively, re-emphasising the importance of homologous in vitro systems.
NOTE
After this manuscript had been submitted, our attention was attracted to the paper by Arnold et al. (1987) describing the isolation of a variant and a pseudogene for human 5S RNA from a genomic DNA library. These genes are transcribed with very low efficiency and these data re-emphasise the importance of obtaining an authentic human 5S RNA gene.
REFERENCES Arnold,
G.J., Kahnt,
B., Herrenknecht,
variant gene and a pseudogene
K. and Gross.
ally active in vitro. Gene 60 (1987) Bieker, T.L., Martin, rate-limiting 40 (1985)
137-144.
P.L. and Roeder,
intermediate
H.J.: A
for 5s RNA are transcriptionFormation
of a
in 5S RNA gene transcription.
R.G.:
Cell
119-127.
Bogenhagen,
D.F. and Brown,
Xenopus 5s DNA required
D.D.: Nucleotide
sequences
for transcription
termination.
S. and Brown,
D.D.:
m Cell
24 (1981) 261-270. Bogenhagen, region
D.F.,
Sakonju,
in the center
initiation
A control
of the 5s RNA gene directs
oftranscription,
specific
II. The 3’ border ofthe region. Ccl1
19 (1980) 27-35. Boulanger,
P.A., Yoshinaga,
properties
and
SK. and Berk. A.T.: DNA-binding
characterization
of human
transcription
factor III C2. J. Biol. Chem. 262 (1987) 1509X-I5 Brownlee,
G.G., Cartwright,
R.: The
nucleotide
E., McShane,
sequence
105.
T. and Williamson,
of somatic
5s
RNA
from
Xenopus laevis. FEBS Lett. 25 (1972) 8-12. Ciliberto,
G., Raugei,
R.: Common
G., Costanzo,
F., Dente,
and interchangeable
of genes transcribed
by RNA
elements
L. and Cortese, in the promoters
polymerase.
Cell 32 (1983)
725-733. Coulombe,
B. and Skup, D.: Expression
interferon-a, mammalian
gene
with
modified
of a synthetic nucleotide
cells. Gene 46 (1986) 89-95.
human
sequence
in
85
Currier,
T.C. and Nester,
circular Biocbem. Doran,
E.W.: Isolation
DNA ofhigh molecular
of covalently
closed
weight from bacteria.
Analyt.
sequences
Bingle,
W.H.
of two human
and
Roy,
K.L.:
The
5S rRNA pseudogenes.
nucleotide Nucl. Acids
Res. 15 ( 1987) 6297. Emerson,
B.M.
arrangement
and
Roeder,
R.C.:
Isolation
of active and inactive
V.A. and Waiters,
and 4.5s (suppl. Forget,
ribosomal
and
genomic
forms of mammalian
SS
B.C. and Weissman, R., Heikens,
synthesis
Nucl.
Res. 14
Acids
S.M.: Nucleotide
Simultaneous fragments: Enzymol.
W., Heisterberg-Moutsis, approach
of KB
G. and Blocker,
of oligonucleotides:
chemical segmental
A., Schwellnus,
synthesis
K. and
and biological
an efficient and complete
Blocker,
applications
H.:
of DNA
methodology.
Methods
M. and Seifart, K.H.: Transcription 5s RNA in a system
in vitro from HeLa cells. Eur. J. Biochem.
of
recon-
117 (1981)
is feedback-inhibited
D., Wingender, for various
formation
for cloning.
Methods
Enzymol.
H.R.B. and Brown, D.D.: A specific transcription
factor
Sci. USA 77 (1980) 4170-4174.
Pieler, T., Hamm,
J. and Roeder.
control
region
ments,
organized
spacing.
is composed
R.G.: The 5S gene internal
of three distinct
as two functional
sequence
domains
ele-
with variable
Cell 48 (1987) 91-100. S., Bogenhagen,
region
in the center
initiation
D.F. and
Brown,
D.D.:
A control
of the 5S RNA gene directs
of transcription,
I. The 5’ border ofthe
specific
region. Ceil
19 {1980) 13-25. F., Nicklen, S. and Coulson,
chain-terminating
inhibitors.
A.R.: DNA sequencing
Proc. Natl. Acad.
with
Sci. USA 74
(1977) 5463-5467. Segall, J., Matsui, RNA polymerase Wingender, lation
T. and Roeder,
for the accurate
R.G.: Multiple
transcription
factors
of purified
are
genes by
III. J. Biol. Chem. 255 (1980) 11986-I 1991.
E., Shi, X.P., Houpert, of a transcription
A. and Seifart,
complex
by HeLa
of 5S RNA genes 5S RNA.
J. Biol.
for ribosomal
K.H.:
Iso-
5S RNA.
K.H.: Transcription
class III genes towards
E., Jahn, D. and Seifart, K.H.: Association
polymerase
III with transcription
L.J. and Brown,
differ in parameters
comof
salt. J. Mol. Biol. 193 (1987)
D.D.: Nucleotide
borealis oocyte
5S DNA: comparison
several
eucaryotic
related
factors
of RNA
in the absence
of
DNA. J. Biol. Chem. 261 (1986) 1409-1413.
E. and Seifart,
and stability
Wingender,
Wormington,
W.M., Bogenhagen,
D.D.: A quantitative scription
sequence of sequences
of Xenopus that flank
genes. Cell 15 (198 1) 1145-l 156.
Communicated
D.F., Jordan,
E. and Brown,
assay for Xert~~pus 5s RNA gene tran-
in vitro. Cell 24 (1981) 809-817.
303-313. Kern,
binding.
EMBO J. 3 (1984) 1761-1768. W. and Seifart, K.H.: Transcription
Chem. 257 (1982) 1468-1472. plexes
and TFHIA
that can bind either the 5S RNA gene or 5S RNA. Proc. Natl.
required
154 (1978) 221-249.
W., Kotzerke,
in vitro Jahn,
on transcription
J.: New Ml3 vectors
Pelham,
Sanger,
Nucl. Acids Res. 11 (1983) 4365-4377.
407-415. Gruissem,
Messing,
Sakonju,
for the simultaneous
the cloned genes for ribosomal stituted
sequence
158 (1967) 1695-1699.
R., Meyerhans,
Gruissem,
5S, 5.8s
sequences.
of large numbers
solid supports,
effects
mutations
5S RNA gene can have
Mol. Cell. Biot. 7 (1987) 486-494.
Acad.
ofpublished
1986) rl-r59.
H.: A new general
Frank,
J.: Collection
RNA
cell 5S RNA. Science Frank.
D.F.: Transition
101 (1983) 20-78.
RNA genes. J. Biol. Chem. 259 (1984) 7916-7925. Erdmann,
G.A. and Bogenhagen,
within the Xenopus borealis somatic independent
76 (1976) 431-441.
J.L.,
McConkey,
by H.G. Zachau.
77
Elsevier GEN 02332
Complete synthesis and transcription (Ribosomal
5s RNA;
III-transcription
in vitro of a gene coding for human rihosomal 5s RNA
gene expression;
in vitro transcription;
HeLa cell extract;
RNA polymerase
III;
Pol
factors)
Edgar Wingender”, Ronald Franka, Helmut Bliicker”, Lingru Wang b, Dieter Jahnb and Klaus H. Seifart’ ‘I Gesellschaft ftir Biotechnologische Forschung, D-3300 Braunschweig (F. R. G.) Tel. 0531/6181206. biologic und Tumorforschung, Philipps-Universitiit, D-3550 Mmburg (F.R. G.) Received
17 November
Accepted
4 December
1987
Received
by publisher
12 January
and Institut ftir Molekular-
1987 1988
SUMMARY
The gene coding for the major human ribosomal 5s RNA was chemically synthesized and cloned into a pUC13 vector. This approach was taken, because attempts to isolate the human 5S gene have thus far yielded either pseudogenes or variant 5s genes of unknown function. The synthetic human gene was transcribed by RNA polymerase III either in a crude HeLa cell extract or in a system reconstituted from partially purified transcription factors. Comparative studies with the Xenopus luevis somatic 5s gene show that the human gene is transcribed with similar fidelity and an efficiency of about 80% under optimal conditions. The time-course of transcription and optimal concentrations of template and transcription factors were found to be similar for both genes studied. The synthetic gene described may prove useful to study its interaction with human transcription
factors
in a homologous
system.
INTRODUCTION
Transcription of the gene for 5s rRNA by RNA polymerase III has proven to be an extremely useful
Correspondence to: Dr. K.H.
Seifart,
biologie und Tumorforschung,
Karl-von-Frisch-Strasse,
Marburg
(F.R.G.)
Abbreviations:
bp, base pair(s); liquid
deoxynucleotide; PMSF,
D-3550
DNA coding
h, human;
polyacrylamide fluoride;
for 5S RNA;
RNA.
I’)88 El.xGx
HEPES.
sulfonic acid; HPLC,
chromatography;
PAGE,
037X-l 119!88~$03.50 0
DTT, dithiothreitol;
N’-2-ethane
phenylmethylsulfonyl
5S DNA,
Rir Molekular-
Tel. 06421-285013.
hydroxyethylpiperazine performance
Institut
oligo,
higholigo-
gel electrophoresis;
TF, transcription 5S rRNA,
factor;
ribosomal
5S
model for the characterisation of the transcription factors involved and for the development of concepts regarding the mechanism of gene regulation in eukaryotic cells. Simultaneously it has become increasingly apparent that the development of homologous systems may be essential for the appropriate characterisation of promoter sequences and factors interacting with them. While TF IIIA, IIIB and IIIC have been isolated and partially purified from human cells (Segall et al., 1980; Wingender et al., 1986; Boulanger et al., 1987) the homologous gene for 5s rRNA has hitherto not been isolated in a transcriptionally active form from genomic DNA. A DNA sequence from a human library, which hybridized to 5s RNA and bound to
Science Publlshcrs B.V. (Bmmcdical Dwision)
78
TF IIIA was not transcribed change in the internal Roeder,
in vitro, due to a base
control
region (Emerson
1984) and it possibly
represents
of a large family of pseudogenes, of unknown
function
(Doran
and
a member
or variant
5S genes
et al., 1987).
In view ofthe outlined necessity to obtain a human 5s rRNA
gene of correct
ficulties associated
library, we synthesized for
the
major
Weissman, homologous
sequence
with its isolation a nucleotide
human
5s
1967) to investigate
and
factors
denaturing
temperatures
conditions
and ligated at
with T4 DNA ligase.
Finally the reaction
products
were checked
by PAGE
(see Fig. 2); all this according
procedures
detailed
elsewhere
(Frank
again to the
et al., 1983;
1987). (b) Cloning and sequencing
sequence coding
rRNA
(Forget
and
its transcription
by a
involved.
Expression of chemically synthesized eukaryotic genes in eukaryotic cells or cell extracts has been hitherto restricted to a few examples of synthetic structural genes due to the complicated and often unknown structure of their promoters. To express a synthetic human interferon-a, gene in murine cells, e.g., these problems were partially circumvented by using a heterologous viral promoter (Coulombe and Skup, 1986). Genes transcribed by RNA polymerase III, however, harbour their own promoters inside the transcribed region. Here we present results showing that a synthetic human 5S rRNA gene is correctly and productively transcribed in an in vitro system reconstituted from a HeLa cellular extract. This proves that for the expression of the human 5S RNA gene, 5’-flanking sequences are not essential, although they might exert additional regulating influences.
MATERIALS
under
the dif-
from a human
cell extract, and to study its interaction
with the transcription
PAGE elevated
AND METHODS
Using
the single-stranded
double
strand
BumHI
protruding
that
were
ends of the synthetic designed
as Sal1
ends, respectively,
gene was cloned into a pUCl3
and
the synthetic
vector. After ligation,
the plasmid was transfo~ed into ~,~~~e~ic~ja coli strain BMH 7 I-18, white clones were selected and checked by restriction analysis. Inserts from the plasmid DNA of positive clones were excised with Hind111 + EcoRI, recloned into phage M13mp18 and sequenced according to Sanger et al. (1977). (c) Preparation of DNA and cellular extracts Biochemicals were reagent grade from Boehringer Mannheim. The plasmids used in this study were isolated in their superhelical form as described (Currier and Nester, 1976) and purified by sucrose density gradient centrifugation. Plasmids pH5S and pX ls5S contained single copies of the synthetic human 5S gene and the X. laevis somatic 5S gene in pUC13 (2797 bp) and pUC I9 (2884 bp), respectively. The cytoplasmic HeLa cell extract (SIOO) was prepared from 20 liter suspension cultures with the titer of 4-5 x lo5 cells/ml, as described previously (Gruissem et al., 1981), and contained approx. 15 mg proteiniml.
(a) Gene design and synthesis Oligodeoxynucleotides comprising basically the coding sequence of the human 5S rRNA, its complementary strand, and ‘sticky ends’ for the restriction enzymes Sal I and BamHI were designed with the SYNGEN option of the GENMON computer programme package (see Fig. 1). synthesised with cellulose disks as segmental supports, purified after deprotection over reversed-phase (disposable cartridges) and ion-exchange (HPLC) materials, labelled at their 5 ’ -termini with [ y-‘*PI ATP and T4 polynucleotide kinase, analysed by sizing on a 20”,
(d) In vitro synthesis and electrophoretic RNA
analyses of
The in vitro transcription reaction mixtures were incubated at 30°C for 1 h unless stated otherwise and contained in a total volume of 50 11 0.025 mM and 10 /iCi [ z-~‘P] GTP (440 Ci/mmol, Amersham), 0.5 mM each of ATP, UTP and CTP 20 mM Tris ’ HCI, pH 7.9, 60 mM KCl, 5 mM MgClz, 3 mM DTT, IO?,; (v/v) glycerol, variable amounts of plasmid DNA and 15 ~1 SlOO. The in vitro transcription products were purified
19
and analyzed acrylamide
by PAGE, gels, and
using 7 M urea-lo”/:, subsequent
poly-
135 or 150 mM
autoradiography
through
overnight as described (Gruissem and Seifart, 1982). The region of the gel containing the RNA was excised
tions fractions
and quantitated
through,
by Cerenkov
radiation.
of transcription
All operations stated
were performed
otherwise.
transcription of HeLa
For
unless
of individual
trated by ammonium
culture
against
(about
B and
stored
at
in preparation).
two consecutive steps of buffer I containing 0.35 M KC1 (fraction B; approx. 1.3 mg protein~ml) and 0.6 M KC1 (fraction C; approx. 0.5 mg protein/ml). Fractions B and C contain TFIIIB and TFIIIC, respectively, and both fractions contain RNA polymerase III. The enzyme was removed from these fractions by dialysing against buffer II (20 mM Tris +HCI, pH 7.9,5 mM MgCl,, 3.0 mM DTT and 0.2 mM PMSF) containing 20% glycerol and either
RESULTS
AND DISCUSSION
(a) Gene synthesis The
chemical
and cloning synthesis
of oligos
as building
blocks for a relatively long DNA duplex comprising a complete gene is most efficiently carried out by simultaneous synthesis of adjacent fragments of
30 I
40 I
3
1
and
dialysed
60 mM KC1 and IO?/;, - 80°C. Human TFIIIA
(hTFIIIA), contained in fraction A (see above) was purified by additional chromatographic steps involving rechromato~aphy on phosphocellulose as will appropriately be published elsewhere (L. W., R. Waldschmidt, D. J., E. W. and K.H. S., manuscript
washed with the same buffer and the flow-through was collected (fraction A; approx. 3.0 mg protein/ml). The column was subsequently eluted with
20 I
sulfate precipitation,
buffer II containing
glycerol
pH 7.9, 3.0 mM DTT, 0.2 mM PMSF, 20% glycerol) containing 0.1 M KCl. The column was
I
III is retained
(Segall et al., 1980). Fractions
at 0-4°C
in suspension
10
RNA-polymerase
in the flow-
nation and from RNA polymerase III, but contained several other proteins. These fractions were concen-
15 mg protein/ml) was applied to a 30 ml; 2.6 x 10 cm phosphocellulose column (Whatman Pl I in its sodium form) in buffer I(20 mM HEPES,
I
bed
Under these condi-
B and C are contained
whereas
passage
C were assayed to be free of mutual cross contami-
the isolation
1
and
protein/ml
factors
factors the SIOO extract from 25 liters
cells grown
sulfate, (1 mg
volume) at these ionic strengths.
on the column (e) Fractionation
~monium
DEAE-Sephadex
50 I
60 I
5
7
TCGACGTCTACGGCCATACCACCCTGAACGCGCCCGATCTCGTCTGATCTC(S’WXT~T~ -TGCCGGTATGGTGGGACTTGCGCGGGCTAGAGCAGACTAGAGCCTTCGAl-KGT2
4
70
80
I
I
90
1
100
110
I
I
11
9 GCCTGGTTAGTACTTWTGGGAGA
..
6
120
I 15
13
CCGCCTGGGMTACCGGGTGCTGTAGGCTTTTAGACTlTTG
CGGACCAATCATGAACCTACCCTCTGGCGGACCCTTATGGCCCACGACATCCGAAAATCTGAAAACCTAG 0
10
Fig. I. Synthesis S. horedis position Sequence
of the human
termination
sequence
5S rRNA gene. Both strands and a BantHI
in the DNA duplex). The overlappings numbering
refers to the transcription
14
12 of the gene for human
site complement
were synthesised
of complementary start point
( = 1).
segments
5S rRNA
as adjacent
were optimised
flanked fragments
by a Sal1 site complement, (numbered
using a computer
according
programme
an
to their
(SYNGEN).
each strand which cover the complete sequence. For optimal hybridisation of complementary fragments
play only a single deviation
prior to their ligation, they have to be properly defined to achieve most stable and unique overlaps.
center
This was achieved the
computer
using an option
programme
package
which runs on VAX computers the operating (Frank For
(SYNGEN)
here, the nontranscribed
structed
of seven,
the transcribed
oligos (Fig. 1). These
fragments
53 which is located
and has recently
been shown
in the
(Pieler et al., 1987) to be important
for
GENMON
and IBM-PC
human
reported
in position
of the boxA homologue
con-
of
SS rRNA strand strand
/
under
systems VMS and DOS, respectively
et al., 1987). synthesis of the
trol region
within the internal
A
I
8
gene
was conof eight
were synthesized
using the filter method, purified and processed as described (Frank et al., 1983; 1987). Analysis of the individual oligos by gel electrophoresis revealed some minor contaminations in an overexposed autoradiograph (Fig. 2A). Nevertheless, they can be efficiently ligated to the correct product in a single reaction step (Fig. 2B) due to their proper design allowing ligation at elevated temperature and, thereby, suppressing any side-reactions. Referring to the nontranscribed strand, the 5’ terminus of the gene was designed to be compatible to a SulI restriction site. The subsequent region coding for the human 5s RNA was taken from the known RNA sequence (Forget and Weissman, 1967; Erdmann and Wolters, 1986). At the 3’ end of this region, the transcription termination sequence of a Xenopus borealis 5s rRNA gene (oocyte-type gene 1; Korn and Brown, 1981) was added which comprises two clusters of four thymidine residues each. These short T-stretches have been shown to represent efficient termination signals for RNA polymerase III transcription (Bogenhagen and Brown, 1981). The 3’ terminus consists of a sequence compatible to a BarnHI restriction site. Thus, the 5s rRNA gene complemented by a termination sequence was suitable to be cloned between the ScllI and the BumHI sites of the vector pUC13 (Messing, 1983). Subsequently, the synthetic gene sequence was verified using the sequencing method of Sanger et al. (1977). This sequence was compared to other 5s RNA genes previously employed for in vitro transcription studies, i.e., the oocyte-type 5s RNA gene from X. borealis (Korn and Brown, 1981) and theX. luevis somatic 5s gene (Brownlee et al., 1972; Fig. 3). The X. Iuevis somatic and the synthetic human gene dis-
m 234m 194mD
'
118c,
721)
1 Fig. 2. (A) Sizing of the synthetic
oligos (in the order
from left to right) on a 20”, polyacrylamide urea; lanes: A, the A ladder
starting
starting
of the one-step
with T,. (B) Analysis
to I5 on a IO”,, non-denaturing sample
of the crude ligation
4O”C, I h at 37”C, markers,
7M
with A,: T, the T ladder ligation of oligos I
polyacrylamide
mixture
I to 15
gel containing
gel; laws:
after incubation
1h at 3O’C, and overnight
(5’-“P-labelled
2
HueHI-fragments
for
I,
I h at
at 15’C; 2, M,
of 4x174).
81
1
20
10
hwn 5s RNA
GTCTACGGCCATACCACCCTGAACGCGCCCGATCTCGTCT l l ******** *********** l l *************
Xls
GCCTACGGCCACACCACCCTGAAAGTGCCCGATCTCGTCT
5s RNA
60
70
80
Xbo 5s RNA
GATCTCGGAAGCGATGCAGGGCCGGGCCTGGTI-AGTACCT l *********** * l ***** ********a****** l
hum 5s RNA
GATCTCGGAAGCTAAGCAGGGTCGGGCCTGGlTAGTACTT l *********** ***************************
Xls
GATCTCGGMGCCAAGCAGGGTCGGGCCTGGlTAGTAClT
5s RNA
90
110
100
120
Xbo 5s RNA
GGATGGGAGACCGCCTGGGAATACCAGGTGTCGTAGGCl-T l ************************ **** ********
hum 5s RNA
GGATGGGAGACCGCCTGGGAATACCGGGTGCTGTAGGClT ******** ********a**************** ****
Xls
GGATGGGAGACCGCCTGGGAATACC
5s RNA
comparison Sequences
AGGTGTCGTAGGCTT
of the gene for human 5s RNA (hum 5s RNA) with the genes for X. borealis oocyte-specific 1981) and for X. laevis somatic
5s RNA; Korn and Brown, by an asterisk.
4.0
GCCTACGGCCACACCCCCCTGAAAGTGCCCGATCTCGTCT l l ******** *** l ****** * **************
50
Fig. 3. Sequence
30
Xbo 5s RNA
of the non-coding
strands
5s RNA (Xls 5s RNA; Brownlee
are given; numbering
et al., 1972). Identical
refers to the transcription
5s RNA (Xbo
residues
are marked
start point ( = 1).
transcription efficiency (McConkey and Bogenhagen, 1987). The oocyte gene promoter differs in this and two additional positions from both these somatic genes.
5s-
(b) Time course of the in vitro transcription of the Xenopus Zuevis somatic and synthetic human SS-genes by a HeLa cell extract A human genomic clone, containing the 5s RNA sequence with one base change in the internal control region was not transcribed in vitro (Emerson
0
J
1
8 2
3
10
5
6
template. times
represent
products
after 5, 10,20,30,45
20
30 Time
45 1min. 1
60
containing counting.
reactions
were stopped
were separated
gels and visualised 5s RNA
insert, part A) or human
*
of the X. /aeviy somatic 5s RNA gene (o--(>). with nucle-
labelled GTP and 20 pg/ml of the indicated
The transcription
and RNA
polyacrylamide l-6
human
HeLa cell extract (SlOO) was incubated
oside triphosphates, 4
for transcription
or the synthetic
Cytoplasmic
-Y
1:
5
Fig. 4. Time course (M)
by autoradiography.
synthesised synthetic
Lanes
from the X. luevis (upper
5s gene (lower insert, part B)
and 60 min, respectively.
5s RNA were excised
at different
on 7 M urea-lo”,
Radioactive
and quantified
bands
by Cerenkov
82
and Roeder, analyse human the
1984). It was therefore
the transcription gene described
established
capacity
of transcription
5s gene. As was previously
(Pelham
and Brown,
scription
of the latter gene displays
to
gene is transcribed product
of the synthetic
here and to compare
kinetics
X. laevis somatic
of interest
it with
Xenopus somatic
of the
thesis
shown
total synthesis
1980; Jahn et al., 1987) trana clear time-lag,
with similar fidelity, yielding
identical
in size to that synthesised
5s gene. The rates of RNA
from both
somewhat
genes
are comparable,
has repeatedly
lower
(about
Figs.
syn-
although
been observed
20%,
a
on the
to be
4 and
5) in
to the Xenopus gene. The reason for this
comparison
presumably due to the delayed incorporation of TFIIIB into the transcription complex (Bieker et al.,
is not clear, but could be attributed to the lack of flanking sequences, possibly modulating the tran-
1985). As shown in Fig. 4, the synthetic
scription
gene
is productively
transcribed
human
in a HeLa
5s cell
extract and the formation of 5s RNA displays a very similar time course, including the time-lag mentioned above. (c) Influence of template concentration To investigate whether the human 5s gene is accepted by transcription factors in the HeLa cell extract with comparable affinity, a DNA titration was conducted in comparison to theX. laevis somatic 5s gene. As is demonstrated
in Fig. 5 the human
ever,
efficiency
that
observed
the
of this gene. It is evident,
DNA-optimum
for transcription
how-
characteristically
of the
5s
gene
and
attributed to the individual dispersion of TFIIIA and TFIIIC to separate genes at high DNA concentration without formation of productive preinitiation complexes (Wingender et al., 1984), is similar for both genes investigated. The absolute position of this optimum is different from that observed for the oocyte-type 5s gene from X. borealis (Gruissem et al., 1981; Jahn et al., 1987). This might be due to several additional base exchanges in the promoter region (50-90) of the latter gene when compared to
l
\ \ 0
\ \ \ \
1
\ \
\ \
\ \
\ \
\ \
\
’\
‘1
‘. \ \\ \
’\
-
a.,
.”
d”
DNA Fig. 5. Transcription GTP and increasing and quantitation
dependency amounts
on template
ofX. luevis (M
were as described
concentration.
&-hnll
HeLa S 100 was incubated
and insert A) or synthetic
in the legend to Fig. 2.
-
for 1 h with nucleotide
human 5s DNA (o-_O
triphosphates,
and insert B). Product
labclled analysis
83
either the X. laevis somatic
or the synthetic
human
gene (Fig. 3) causing less stable protein-DNA
inter-
actions
(Wormington
et al., 198 1).
(d) Influence of TFIIIA Binding of TFIIIA
and TFIIIC
from HeLa cells
to the internal
control region of
the 5s gene is the primary event for the formation transcription
complexes
on this gene. Although
of the
exact function of TFIIIC in this context is still not fully understood, recent investigations by Pieler et al. (1987) have demonstrated
interactions
of this factor
with boxA and probably also with boxC of the internal control region. It was therefore important to analyse the effect ofthese factors on the transcription
Fig. 6. Titration stituted
of the synthetic human 55 gene. It was found (Fig. 6) that 5S RNA synthesis from both genes increases with rising concentrations ofhTFIIIA up to a certain point and then decreases with very high concen-
genes in question. A comparable optimum is not observed for the titration of hTFIIIC (Fig. 7). It was observed that rising hTFIIIC concentrations increased 5s RNA formation without a subsequent decline. As is shown in Fig. 7, maximal rates of 5S RNA synthesis are
Fig. 7. Titration
of increasing
amounts
RNA gene (part B). Transcription ofTFIll.A,
10.0 ,ul ofTFIIIB,
The amounts
of hTFIIIf
of hTFIItC
factors
in a reconstituted
were
purilied
AND
METHODS,
TFIIIC,
varying amounts
template
were incubated
hTFIIIA
employed
ofTFIIIC
amounts
of hTFIIIA
respectively.
from
HeLa
in a recon-
(part A) OF synthetic ceils
factors as
IIIA, IIIB
described
section e. Ten yl ofTFIIIB, ofTFIIIA for
in
IO ~1 of
and 10 p’g DNA/ml
of either
1h in all assays. The amounts
of
were: in part A (lanes 1-5) O.OS,O.I, 0.5. 1.0,
5.0 ~1, respectively,
and in part B (lanes l-4) 0.05,0.5,
Quantitation
I .O. 5.0 ~1,
of 5s RNA was as in Fig. 2.
possibly reached at lower concentrations of/zTFIIIC in the case of the Xenopus gene. Footprint analyses (not shown; manuscript in prep~ation) proved, however, that hTFIIIC has little or no effect on the affinity of hTFIIIA binding to the human gene.
system with the X. iuevis somatic
were purified from HeLa celis as described
varying concentrations employed
IIIC
MATERIALS
trations of hTFIIIA. The basic phenomenon is similar for both genes, although the exact position of the optimum is slightly different, which could indicate an altered interaction of this factor with the two
of increasing
with the X. lnevis somatic
5s RNA gene (part B). Transcription
human and
system
and 5 ,ugjml ofeither
in
MATERIALS
DNA template
were 0.1, 0.5, 1, 2.5, 5, 7.5. 10, 20 and 50~1 in lanes
l-9,
(part A) or synthetic AND
METHODS,
were incubated
respectively.
human
5s
section e. One iti for 1 h in all assays.
84
(e) Conclusions
ACKNOWLEDGEMENTS
A gene coding for the major human chemically
synthesized.
5S rRNA was
This gene deviates
X. luevis somatic 5s gene, frequently studies, in eight positions.
from the
used for in vitro
One of them (at position
53) is located within the A box of the internal
control
region (Pieler et al., 1987). Although in a degenerate position of the BoxA consensus sequence, derived from either the tRNA genes (Ciliberto eukaryotic
5s RNA sequences
is apparently
important
We
acknowledge
Deutsche
financial
support
Forschungsgemeinschaft
conducted
at the University
of
the
to the research
of Marburg
and the
expert technical assistance of Frauke Seifart, Ursula Kopiniak and Verena Buckow (Marburg) as well as Helga Krause,
Christiane
Giesa,
Wiebke
Heikens
and Heiko Mielke (Braunschweig).
et al., 1983) or
(Pieler et al., 1987), it
for transcription
efficiency
(McConkey and Bogenhagen, 1987). However, we did not observe enhanced transcription as reported by these authors for a CG-TA transition in that position of the X. borealis somatic 5s gene. Our results clearly show that the synthetic human 5S rRNA gene is correctly and efficiently transcribed by RNA polymerase III either in a crude HeLa cell extract or in a reconstituted system of partially purified transcription factors. This proves that flanking regions are not required for transcription of the human 5S gene as was previously shown for the X. borealis somatic gene (Bogenhagen et al., 1980; Sakonju et al., 1980). Nevertheless, these flanking sequences may exert either positively or negatively modulating influences, as has recently been shown for some point mutations in the upstream region of that gene by McConkey and Bogenhagen (1987). Differences in the flanking sequences between the genes compared in this study may account for the slightly lower transcription efficiency of the synthetic human gene (approx. 80% under optimal conditions) and may possibly overcome the otherwise positive C + T transition at position 53. The synthetic gene described may prove useful to study its interaction with human transcription factors in a homologous system. We are presently analysing whether the small differences observed in the factor concentrations required for optimal transcription of the two genes could reflect altered protein-DNA interactions. Preliminary results from comparative footprint experiments show an altered interaction of human TFIIIA with the human and X. laevis somatic 5S genes, respectively, re-emphasising the importance of homologous in vitro systems.
NOTE
After this manuscript had been submitted, our attention was attracted to the paper by Arnold et al. (1987) describing the isolation of a variant and a pseudogene for human 5S RNA from a genomic DNA library. These genes are transcribed with very low efficiency and these data re-emphasise the importance of obtaining an authentic human 5S RNA gene.
REFERENCES Arnold,
G.J., Kahnt,
B., Herrenknecht,
variant gene and a pseudogene
K. and Gross.
ally active in vitro. Gene 60 (1987) Bieker, T.L., Martin, rate-limiting 40 (1985)
137-144.
P.L. and Roeder,
intermediate
H.J.: A
for 5s RNA are transcriptionFormation
of a
in 5S RNA gene transcription.
R.G.:
Cell
119-127.
Bogenhagen,
D.F. and Brown,
Xenopus 5s DNA required
D.D.: Nucleotide
sequences
for transcription
termination.
S. and Brown,
D.D.:
m Cell
24 (1981) 261-270. Bogenhagen, region
D.F.,
Sakonju,
in the center
initiation
A control
of the 5s RNA gene directs
oftranscription,
specific
II. The 3’ border ofthe region. Ccl1
19 (1980) 27-35. Boulanger,
P.A., Yoshinaga,
properties
and
SK. and Berk. A.T.: DNA-binding
characterization
of human
transcription
factor III C2. J. Biol. Chem. 262 (1987) 1509X-I5 Brownlee,
G.G., Cartwright,
R.: The
nucleotide
E., McShane,
sequence
105.
T. and Williamson,
of somatic
5s
RNA
from
Xenopus laevis. FEBS Lett. 25 (1972) 8-12. Ciliberto,
G., Raugei,
R.: Common
G., Costanzo,
F., Dente,
and interchangeable
of genes transcribed
by RNA
elements
L. and Cortese, in the promoters
polymerase.
Cell 32 (1983)
725-733. Coulombe,
B. and Skup, D.: Expression
interferon-a, mammalian
gene
with
modified
of a synthetic nucleotide
cells. Gene 46 (1986) 89-95.
human
sequence
in
85
Currier,
T.C. and Nester,
circular Biocbem. Doran,
E.W.: Isolation
DNA ofhigh molecular
of covalently
closed
weight from bacteria.
Analyt.
sequences
Bingle,
W.H.
of two human
and
Roy,
K.L.:
The
5S rRNA pseudogenes.
nucleotide Nucl. Acids
Res. 15 ( 1987) 6297. Emerson,
B.M.
arrangement
and
Roeder,
R.C.:
Isolation
of active and inactive
V.A. and Waiters,
and 4.5s (suppl. Forget,
ribosomal
and
genomic
forms of mammalian
SS
B.C. and Weissman, R., Heikens,
synthesis
Nucl.
Res. 14
Acids
S.M.: Nucleotide
Simultaneous fragments: Enzymol.
W., Heisterberg-Moutsis, approach
of KB
G. and Blocker,
of oligonucleotides:
chemical segmental
A., Schwellnus,
synthesis
K. and
and biological
an efficient and complete
Blocker,
applications
H.:
of DNA
methodology.
Methods
M. and Seifart, K.H.: Transcription 5s RNA in a system
in vitro from HeLa cells. Eur. J. Biochem.
of
recon-
117 (1981)
is feedback-inhibited
D., Wingender, for various
formation
for cloning.
Methods
Enzymol.
H.R.B. and Brown, D.D.: A specific transcription
factor
Sci. USA 77 (1980) 4170-4174.
Pieler, T., Hamm,
J. and Roeder.
control
region
ments,
organized
spacing.
is composed
R.G.: The 5S gene internal
of three distinct
as two functional
sequence
domains
ele-
with variable
Cell 48 (1987) 91-100. S., Bogenhagen,
region
in the center
initiation
D.F. and
Brown,
D.D.:
A control
of the 5S RNA gene directs
of transcription,
I. The 5’ border ofthe
specific
region. Ceil
19 {1980) 13-25. F., Nicklen, S. and Coulson,
chain-terminating
inhibitors.
A.R.: DNA sequencing
Proc. Natl. Acad.
with
Sci. USA 74
(1977) 5463-5467. Segall, J., Matsui, RNA polymerase Wingender, lation
T. and Roeder,
for the accurate
R.G.: Multiple
transcription
factors
of purified
are
genes by
III. J. Biol. Chem. 255 (1980) 11986-I 1991.
E., Shi, X.P., Houpert, of a transcription
A. and Seifart,
complex
by HeLa
of 5S RNA genes 5S RNA.
J. Biol.
for ribosomal
K.H.:
Iso-
5S RNA.
K.H.: Transcription
class III genes towards
E., Jahn, D. and Seifart, K.H.: Association
polymerase
III with transcription
L.J. and Brown,
differ in parameters
comof
salt. J. Mol. Biol. 193 (1987)
D.D.: Nucleotide
borealis oocyte
5S DNA: comparison
several
eucaryotic
related
factors
of RNA
in the absence
of
DNA. J. Biol. Chem. 261 (1986) 1409-1413.
E. and Seifart,
and stability
Wingender,
Wormington,
W.M., Bogenhagen,
D.D.: A quantitative scription
sequence of sequences
of Xenopus that flank
genes. Cell 15 (198 1) 1145-l 156.
Communicated
D.F., Jordan,
E. and Brown,
assay for Xert~~pus 5s RNA gene tran-
in vitro. Cell 24 (1981) 809-817.
303-313. Kern,
binding.
EMBO J. 3 (1984) 1761-1768. W. and Seifart, K.H.: Transcription
Chem. 257 (1982) 1468-1472. plexes
and TFHIA
that can bind either the 5S RNA gene or 5S RNA. Proc. Natl.
required
154 (1978) 221-249.
W., Kotzerke,
in vitro Jahn,
on transcription
J.: New Ml3 vectors
Pelham,
Sanger,
Nucl. Acids Res. 11 (1983) 4365-4377.
407-415. Gruissem,
Messing,
Sakonju,
for the simultaneous
the cloned genes for ribosomal stituted
sequence
158 (1967) 1695-1699.
R., Meyerhans,
Gruissem,
5S, 5.8s
sequences.
of large numbers
solid supports,
effects
mutations
5S RNA gene can have
Mol. Cell. Biot. 7 (1987) 486-494.
Acad.
ofpublished
1986) rl-r59.
H.: A new general
Frank,
J.: Collection
RNA
cell 5S RNA. Science Frank.
D.F.: Transition
101 (1983) 20-78.
RNA genes. J. Biol. Chem. 259 (1984) 7916-7925. Erdmann,
G.A. and Bogenhagen,
within the Xenopus borealis somatic independent
76 (1976) 431-441.
J.L.,
McConkey,
by H.G. Zachau.